Potentially pathogenic culturable bacteria in hemodialysis waters

Background Hemodialysis patients are at risk of acquiring healthcare-related infections due to using non-sterile water to prepare hemodialysis fluid. Therefore, microbiological control and monitoring of used water are of crucial importance. Materials and methods In this work, we identified bacterial populations occupying a hemodialysis water distribution system for almost a 6-month period in Ahvaz city, southwest of Iran. A total of 18 samples from three points were collected. We found high colony counts of bacteria on R2A agar. 31 bacteria with different morphological and biochemical characteristics were identified by molecular-genetic methods based on 16 S rRNA gene sequencing. Endotoxin concentrations were measured, using Endosafe® Rapid LAL Single-Test Vials. Results A diverse bacterial community was identified, containing predominantly Gram-negative bacilli. The most frequently isolated genus was Sphingomonas. Five species including M. fortuitum, M. lentiflavum, M.szulgai, M. barrassiae, and M. gordonae was identified .Despite the presence of Gram-negative bacteria the endotoxin analysis of all samples revealed that their endotoxin values were below the detection limit. Conclusion The members of Sphingomonas genus along with Bosea and mycobacteria could be regarded as pioneers in surface colonization and biofilm creation. These bacteria with others like Pelomonas, Bradyrhizobium, staphylococcus, and Microbacterium may represent a potential health risk to patients under hemodialysis treatment.


Introduction
End-stage kidney disease (ESKD) is a significant public health problem worldwide.Patients with ESKD suffer from a systemic impairment, and the direct effect of uremic conditions and its metabolic outcomes makes them more susceptible to infection.These disorders include abnormalities of neutrophils, lymphocytes B, Hemodialysis (HD) is a renal replacement therapy for ESKD patients.This technique is based on the use of an artificial kidney (dialyzer) that removes nitrogenous waste products from the blood by diffusion and unwanted water by ultrafiltration [6].During an average week of hemodialysis, a patient can be exposed to 300-600 L of water, providing multiple opportunities for potential patient exposure to waterborne pathogens [7].
Therefore, hemodialysis water treatment requires softening, carbon filtration, reverse osmosis, and deionization before it can be used [7].Bacteriostatic agent, chlorine, which is added for disinfection of drinking water, gets removed from dialysis water during water treatments.This makes the water susceptible to bacterial proliferation [8].Therefore, bacterial contamination of the dialysis water and dialysate may cause biofilm (glycocalyces) formation and release of endotoxins in the Hemodialysis system [7].Endotoxins (ET) are heatstable lipopolysaccharides (LPS) and the major cell wall components of Gram-negative bacteria.The molecular mass of LPS ranges between 2,000 and 20,000 Da.LPS can be transferred through membranes with large pore sizes by back filtration/diffusion from the dialysis fluid to the blood compartment [9].HD water quality control is a public health problem on a worldwide scale, with quality standards being recommended in all countries.The European Renal Association (ERS) recommends values of ≤ 100 colony-forming units (CFU)/ml of viable bacteria and ≤ 0.5 IU/ml ET as safety criteria for hemodialysis fluid [10].The Japanese Society for Dialysis Therapy (JSDT) recommends a count of viable bacterial cells of Less than 100 CFU/mL, and a maximum of 0.05 EU / mL of ET [11].
According to the American Association for the Advancement of Medical Instrumentation (AAMI), the maximum count limit for heterotrophic bacteria is 100 CFU/mL, and 0.25 EU/mL for endotoxin [12].The reason behind these strict restrictions is that bacteremia and chronic inflammation may contribute to morbidity and mortality [7].
However, despite these strict standards, waterborne outbreaks in the hemodialysis setting continue to occur.Nevertheless, periodic microbial control conducted at hemodialysis center's do not include analysis of nontuberculous mycobacteria (NTM), and there are few published reports on the isolation and identification of these organisms.Currently, there is a growing interest in NTM disease as a result of the association of NTM infections with immune-suppression [13].
The aim of this study was to investigate the bacteriological quality of the hemodialysis water used at a public hemodialysis center in Ahvaz city, southwestern Iran by isolating and identifying the Gram-negative and Grampositive bacteria and NTM.

Water samples collection
This cross-sectional study was conducted for 6 months, from April 2019 to September 2019, at a public hemodialysis center in Ahvaz, Southwest Iran.A total of 18 samples were collected.Three points were selected for sampling: municipality water reservoir stock (point1), water softener (point2), and Outlet of RO equipment (point3) (Fig. 1).Two samples (500 ml) were collected separately for bacterial and Mycobacterium cultures at each time point.In addition, the samples for ET analysis (10 mL of water) were collected aseptically in pyrogenfree glass bottles with a screw cap.

Endotoxin detection
Endotoxin concentrations were measured, using Endo-safe® Rapid LAL Single-Test Vials (STV) containing gel-clot Limulus amebocyte lysate (LAL) (Charles River Laboratories, USA).Aseptically added directly 0.2 mL of sample into LAL assay tube; gently mixed.Immediately placed the reaction tubes in a 37 °C water bath for 60 min.Recorded results by inverting the tube 180 degrees for firming gel.A positive product control was used by the kit.

Bacterial culture and strain isolation
Briefly, 0.1 ml of each sample was pipetted and inoculated on Reasoner's 2 A agar plates (R2A; Merck, Germany) and incubated at 22 °C for 7 days.The number of colonies obtained was multiplied by 10 to obtain the CFU/ml.For NTM Isolation, 500 ml of each sample was filtered through a 0.45-µm pore size membrane filter (Millipore, Bedford, U.S.A) and decontaminated using 0.005% cetylpyridinium chloride (CPC) (30 min in room temperature).The sediment obtained after centrifugation was suspended in 2 mL of phosphate-buffered saline (PBS) and inoculated into two Löwenstein -Jensen (LJ) media (HiMedia, India), and incubated at 37 and 25 °C for 2 months [14].The cultures were monitored weekly to observe colony growth, morphology, and pigmentation.Grown colonies were stained by the Ziehl-Neelsen technique to highlight the presence of acid-fast bacilli.Phenotypical and biochemical tests accompanied by 16 S rRNA sequence analysis techniques were used to identify the acid-fast bacilli.

Bacterial isolates identification and characterization
Each of the isolates was observed for the colony morphological characters such as color, size, shape, transparency, texture, and margin.Homogeneous-looking colonies were collected and propagated.Microscopic features were determined through Gram staining.

Biochemical characterization
The pure cultures isolates were differentiated by various biochemical characteristics such as catalase and oxidase reaction, citrate utilization, urea hydrolysis, indole and H2S production.Based on the morphological examination and biochemical assays, all obtained pure cultures were classified into the genera and identified to the species according to 16 S rRNA Sequencing.

Molecular identification using 16 S rRNA sequencing
The genomic DNA of isolated bacteria was extracted using QIAamp DNA Mini Kit (Qiagen, Germany) according to the manufacturer's instructions.Furthermore, the 16SrRNA gene amplification and sequencing were carried out via the following universal primers: fD1 (5´-AGA GTT TGA TCC TGG CTC AG-3´) and rD1 (5´-AAG GAG GTG ATC CAG CC-3´) [15].Each reaction was run with a 50 ml mix using I-Taq Maxime PCR Premix (iNtRON Biotechnology, Korea).PCR was conducted via the conditions described previously [16].PCR-amplified products of about 1450 bp were obtained from the 16 S rDNA of all the strains.In all stages of DNA extraction and PCR, sterile distilled water was used as a negative control and Escherichia coli strain K-12 (ATCC 10,798) was used as a positive control.The amplicons were sequenced in both directions by an external service (bioneer Inc, South Korea).All sequences were edited and assembled using DNA Sequence Assembler v4 (2013).Partial 16 S rRNA sequences were compared with the sequences available in the NCBI database (http://www.ncbi.nlm.nih.gov) using BLASTN [17,18].Evolutionary analysis was carried out in MEGA6 based on the Maximum Likelihood algorithm with the Kimura-2-parameter model [19,20] and 1000-bootstrap replication.Isolates were assigned to a species when their 16 S rRNA gene sequences were at least 99% identical to a reference isolate clearly.

Results
We found high colony counts of bacteria on R2A agar.All 18 samples presented positive cultures and the number of culturable bacteria increased from the municipal reservoir (point 1) to the dialysis fluid outlets (point 3).The mean colony count in each point was respectively 2.2 × 10 2 , 7.1 × 10 2 , and 10.5 × 10 2 CFU/mL.Gram staining results showed that Gram-negative bacilli were dominant in all samples (61.3%), but faecal coliforms were not detected.Based on the phenotypic characteristics, they were classified into groups and one isolate from each group was randomly selected for or 16 S rRNA gene sequencing.Out of 18 samples from all locations at the HD centre, 31 isolates (19 Gram-negative, 7 Gram-positive and 5 NTM) were studied.At least one Gram-negative isolate could not be identified even by the 16 S rRNA gene sequencing analysis.According to the 16 S rRNA gene sequencing analysis (Fig. 2), the most frequently isolated genus was Sphingomonas (in terms of number and variety).
Unlike Gram-negative bacteria, the number and variety of Gram-positive bacteria were low and limited to three genera.A total of 11 NTM suspected isolates from all three points were included in the study.These isolates were identified on the basis of growth conditions, biochemical characters, and the sequence analysis of the 16s Fig. 2 Phylogenetic tree of 16s rRNA sequences.The evolutionary distances were computed using the Kimura 2-parameter method with 1000 bootstrap replication.Phylogenetic analyses were conducted in MEGA6.Closed circles (•) indicate the out-group rRNA.Ten confirmed sequences belonged to five species including M. fortuitum, M. lentiflavum, M.szulgai, M. barrassiae, and M. gordonae.The infectious potential of isolates in humans is listed in Tables 1, 2 and 3. Nevertheless, it is important to mention that the phylogeny of the 16 S rRNA gene is not accurate for species identification in this genus.
Despite the presence of Gram-negative bacteria, the endotoxin analysis of all samples revealed that their endotoxin values were below the detection limit.

Discussion
Hemodialysis is an alternative therapy for patients with chronic renal failure, increasing the quality and quantity of life of these patients.The quality of the hemodialysis water is of paramount importance in ensuring patient safety [11,52].
In the present study, we assessed the quality of the main and treated water used at a public hemodialysis center in Ahvaz, Iran.The dialysis department at the public hospital in Ahvaz is a major regional center handling a high volume of cases.It is one of the largest facilities in the southwest, serving around 400 patients monthly across three daily shifts.The patient load comprises emergency admissions, local chronic cases, and patients from other cities, and those with advanced kidney disease, diabetes, cancer, including both men and women.There are reports of the presence of nontuberculous mycobacteria (NTM) strains in major parts of the water supplies at hospitals in Ahvaz, which could potentially serve as a source for nosocomial infections [53].Originally, the authors discovered through their literature review that water-source infections were a known issue.However, they found that no previous study had specifically focused on isolating and investigating these infections across different environments.This gap in research, especially in specialized settings like the one they were examining, motivated the authors to conduct their own study to fill this knowledge gap and shed light on the topic.
Investigating the microbiological quality of water requires attention to the type of culture medium, incubation temperature and incubation time.Furthermore, hospital waters are highly oligotrophic habitats and bacteria have adapted their metabolic characteristics to this environment [54], so in order to isolate these bacteria, we use Reasoner's 2 A agar, a low-nutrient culture medium, an incubation temperature of around 22 °C and an incubation period of 7 days for detecting viable bacterial counts in hemodialysis water as a standard method approved by the United States and the European Pharmacopoeia [55,56].
The findings of this study demonstrate a diverse microbial community of bacteria in HD water.Gram-negative bacteria are the major contaminants of water in hemodialysis units as reported elsewhere [54,57] as seen in the results (Table 1).
Although the microbiological quality of municipal water that flows to the hemodialysis center met drinking water regulations [7], removing the bacteriostatic agent chlorine from the dialysis water makes it susceptible to bacterial proliferation [58] therefore in line with other studies [58,59], we observed an increase in culturable bacteria from the municipal reservoir to the dialysis fluid outlets.Rapid, rapid growing mycobacteria (< 7 days); slow, Slow growing mycobacteria (≥ 7 days); * Mycobacterium szulgai (photochromogenic when grown at 24 degrees and scotochromogenic at 37 degrees) Y, yellow; O, Orange; Y-O, yellow-orange, The most abundant and diverse isolates belonged to the family Sphingomonadaceae (Sphingomonas and Sphingobium).Members of this family are strictly aerobic with a characteristic yellow pigmentation.The capacity of sphingomonads to adapt to the human-engineered environments is remarkable.For instance, they are able to survive in chlorinated water and produce biofilms.Due to the fact that sphingomonads are opportunistic pathogens [21,26,28,[60][61][62], their ubiquity and abundance are potentially hazardous, mainly in hospital waters.
Another bacteria that were identified in abundance was Bosea species.Members of the genus Bosea are Mn (II)-oxidizing bacteria [63].Methylobacteria was another Mn (II)-oxidizing bacteria isolated in this study.Evidence shows that Methylobacteria survive and even grow in sterile autoclaved water [64].Biogenic Mn oxides have strong oxidative characteristics and rapidly oxidize other metals, such as chromium and arsenic, which affects their speciation, solubility, and toxicity.In addition to their strong redox activity, Mn oxides degrade refractory organic compounds, which may affect the growth of microorganisms in water distribution systems [65].On the other hand, studies showed that compared with healthy controls, HD patients have significantly higher blood levels of some heavy metals like lead, arsenic and cadmium [66,67].It is possible that there may be a relationship between the high levels of heavy metals in the body of hemodialysis patients and the presence of Mnoxidizing bacteria in the dialysis water.Furthermore, Bosea and Methylobacterium species were previously documented as opportunistic pathogens in humans.Bosea massiliensis isolated in this research have been reported from intensive care unit (ICU) patients [22].Other Bosea species cause eye infection [68], central venous catheter infection and bacteremia [22].Methylobacterium species have been involved in immunocompromised patients and are frequently isolated from blood, liquor cerebrospinalis, bone marrow, synovia, and ascitic and peritoneal fluids.Also, methylobacterium pseudo-outbreaks after endoscopic and bronchoscopy procedures have been related to contaminated tap water [69,70].
This study has provided five NTM species which are potentially pathogenic (Table 3).The most prevalent species was M. fortuitum followed by M. gordonae.This was in agreement with the findings of the study conducted by Roshdi Maleki et al. in the northwest of Iran [71].
The findings show that hemodialysis water can be considered a reservoir for NTM.Cell surface hydrophobicity is a major determinant of the survival and proliferation of NTM in water distribution systems.Also, NTM can survive within Free-living amoeba (FLA), like Acanthamoeba [72].The presence of amoebae in dialysis water has been proven [73].FLA in water are hosts to many bacterial species living in such an environment [74] like Mycobacterium, Variovorax, Bosea, and Acidovorax [75] that were found in this study.Since many of the pathogenic and potentially pathogenic bacteria which interact with FLA are water-borne there is a clear risk for hemodialysis patients.
In this study we have isolated some slime-forming bacteria, like Sphingomonas [87] and Bosea [88] produce extracellular complex carbohydrates and play an essential role in biofilm establishment.NTM also have high cell surface hydrophobicity, which facilitates the formation of biofilms [89].These three types of bacteria were identified as being the most common genera in the present study and could be considered pioneers in colonizing surfaces and creating biofilm communities.Remarkably, sphingomonas and mycobacterium were found in all three sampling points, an indication of their predominant role of them in the bacterial community.
The microbiological quality of water in dialysis units is critically dependent upon the presence of biofilm in the distribution network.Stagnation and high water temperature in the dialysis machine cause microbiological growth and biofilm formation in the dialysis system pipes.An endotoxin-free dialysate does not exclude the risks and hazards of bacteria and an endotoxin discharge from the biofilms, which may have developed on the fluid pathway tubing, may act as a reservoir for continuous contamination.
According to the current guidelines characterization of bacterial communities in hemodialysis water is usually limited to the total viable count.
However, based on the information provided, there are several potential impacts and ways this survey could help the hospital:

Fig. 1
Fig. 1 Schematic of water treatment system and points of sampling

1 .
Identifying Potential Pathogens: The survey identified opportunistic bacteria like Sphingomonas, Bosea, Methylobacterium, and NTM species.This knowledge allows the hospital to target these organisms in their surveillance efforts, potentially leading to earlier detection and improved patient care.2. Tailoring Disinfection Protocols: Understanding the specific bacterial communities present allows for more targeted disinfection strategies.The hospital can choose methods that effectively address the identified organisms within their water system.3. Mitigating Biofilm Risks: The presence of Sphingomonas highlights the importance of biofilm management.The hospital can implement protocols to disrupt and remove biofilms, preventing them from becoming a persistent source of contamination.4. Identifying Environmental Reservoirs: Finding NTM and other opportunistic pathogens suggests the water system as a potential reservoir for hospital-acquired infections.This awareness can guide targeted interventions to minimize risks for vulnerable patients.5. Benchmarking Future Monitoring: This survey serves as a baseline for future monitoring.The hospital can track changes in bacterial populations over time and assess the effectiveness of any implemented interventions.6. Informing Policy Updates: The recommendation to revisit evaluation methods aligns with potential policy updates by public health authorities.This survey's findings can contribute to improving overall water quality standards in hemodialysis settings.

Table 1
Some characteristics of all Gram-negative isolated bacteria and their related human infections

Table 2
All Gram-positive isolated bacteria from dialysis system and their related human infections R, Rod; C, Cocci Y, Yellow; YW, Yellow-White; PO, Pink-Orange; ND, Not Diagnosis.

Table 3
Nontuberculous mycobacteria (NTM) isolated from dialysis system and their related human infections